Targeted deletion or pharmacological inhibition of MMP-2 prevents cardiac rupture after myocardial infarction in mice
Shin-ichiro Matsumura, Shiro Iwanaga, Satsuki Mochizuki, Hiroyuki Okamoto, Satoshi Ogawa, Yasunori Okada
Shin-ichiro Matsumura, Shiro Iwanaga, Satsuki Mochizuki, Hiroyuki Okamoto, Satoshi Ogawa, Yasunori Okada
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Article Cardiology

Targeted deletion or pharmacological inhibition of MMP-2 prevents cardiac rupture after myocardial infarction in mice

Abstract

MMPs are implicated in LV remodeling after acute myocardial infarction (MI). To analyze the role of MMP-2, we generated MI by ligating the left coronary artery of MMP-2–KO and WT mice, the latter of which were administered orally an MMP-2–selective inhibitor or vehicle (TISAM). The survival rate was significantly higher in MMP-2–KO and TISAM-treated mice than in control WT mice. The main cause of mortality in control WT mice was cardiac rupture, which was not observed in MMP-2–KO or TISAM-treated mice. Control WT mice, but not MMP-2–KO or TISAM-treated mice, showed activation of the zymogen of MMP-2, strong gelatinolytic activity, and degradation of ECM components, including laminin and fibronectin, in the infarcted myocardium. Although infarcted cardiomyocytes in control WT mice were rapidly removed by macrophages, the removal was suppressed in MMP-2–KO and TISAM-treated mice. Macrophage migration was induced by the infarcted myocardial tissue from control WT mice and was inhibited by treatment of macrophages with laminin or fibronectin peptides prior to migration assay. These data suggest that inhibition of MMP-2 activity improves the survival rate after acute MI by preventing cardiac rupture and delays post-MI remodeling through a reduction in macrophage infiltration.

Authors

Shin-ichiro Matsumura, Shiro Iwanaga, Satsuki Mochizuki, Hiroyuki Okamoto, Satoshi Ogawa, Yasunori Okada

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Inflammatory cell accumulation and angiogenesis in boundary areas of the...
Inflammatory cell accumulation and angiogenesis in boundary areas of the infarcted myocardium evaluated by immunohistochemistry. Frozen sections were immunostained for CD68, Mac-3, and CD45, and we determined accumulation of immunoreactive cells, denoted as cells/mm2, by counting immunoreactive cells in 5 different areas of 0.25 mm2 using NIH Image software as described in Methods. Similarly, paraffin sections were immunostained for vWF and immunoreactive blood vessels with an apparent luminal area were counted. (A and B) Infiltration of CD68- or Mac-3–immunoreactive macrophages in infarcted myocardium from vehicle-treated control WT, TISAM-treated, and MMP-2–KO mice on days 1, 3, 7, and 14. (C) Infiltration of CD45-reactive polymorphonuclear leukocytes in infarcted myocardium from control WT, TISAM-treated, and MMP-2–KO mice on days 1, 3, 7, and 14. (D) Angiogenesis in infarcted myocardium from control WT, TISAM-treated, and MMP-2–KO mice on days 1, 3, 7, and 14. *P < 0.05; **P < 0.01; ***P < 0.001.